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首页> 外文期刊>The Journal of Horticultural Science & Biotechnology >In vitro production of true-to-type plants of Vitex negundo L. from nodal explants
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In vitro production of true-to-type plants of Vitex negundo L. from nodal explants

机译:用节点外植体体外生产真叶荆条的真型植物

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摘要

An efficient micropropagation protocol, involving axillary bud multiplication, was established to clone Vitex negundo L. plants. An optimum regeneration frequency (97%) and a desirable organogenic response, in the form of multiple shoots, was obtained on Murashige and Skoog (MS) medium augmented with 5.0 mu M 6-benzyladenine (BA) in combination with 0.5 mu M 1-naphthaleneacetic acid (NAA). Healthy, growing in vitro-raised microshoots rooted efficiently on MS medium supplemented with 1.0 mu M indole-3-butyric acid (IBA). Following standard hardening procedures, rooted shoots were transferred to the field with >= 90% survival. No morphological variations were detected among the micropropagated plants when compared with the mother plant. Inter-simple sequence repeat (ISSR) markers were used to evaluate the genetic stability of both the in vitro and in vivo propagated plants. All ISSR profiles from micropropagated plants were monomorphic, and similar to those of field-grown control plants. These results suggest that the culture conditions used for axillary bud proliferation are appropriate for clonal propagation of this medicinally important plant as they do not appear to interfere with the genetic integrity of in vitro -regenerated plants (i.e., no somaclonal variation).
机译:建立了一种有效的微繁殖方案,该方案涉及腋芽繁殖,以克隆Vitex negundo L.植物。在Murashige和Skoog(MS)培养基上添加5.0μM 6-苄基腺嘌呤(BA)和0.5μM 1-的组合,获得了最佳的再生频率(97%)和理想的器官发生反应(多发芽形式)。萘乙酸(NAA)。健康,成长的体外培养的微枝有效地扎根于补充了1.0μM吲哚-3-丁酸(IBA)的MS培养基上。按照标准的硬化步骤,将生根的芽以> = 90%的存活率转移到田间。与母本植物相比,在微繁殖的植物中未检测到形态变化。简单序列间重复(ISSR)标记用于评估体外和体内繁殖植物的遗传稳定性。来自微繁殖植物的所有ISSR图都是单态的,与田间生长的对照植物相似。这些结果表明,用于腋芽增殖的培养条件适合于该药用重要植物的克隆繁殖,因为它们似乎不干扰体外再生植物的遗传完整性(即无体细胞克隆变异)。

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